1740
J. Nat. Prod. 2004, 67, 1740-1743
Phytochemical Studies on Stemona burkillii Prain: Two New Dihydrostemofoline Alkaloids Pitchaya Mungkornasawakul,†,‡ Stephen G. Pyne,*,† Araya Jatisatienr,§ Wilford Lie,† Alison T. Ung,† Kritchaya Issakul,§ Auntika Sawatwanich,§ Damrat Supyen,⊥ and Chaiwat Jatisatienr§ Department of Chemistry, University of Wollongong, Wollongong, New South Wales, 2522, Australia, Division of Environmental Sciences, Chiang Mai University, Chiang Mai 50202, Thailand, Department of Biology, Chiang Mai University, Chiang Mai 50202, Thailand, and Department of Chemistry, Chiang Mai University, Chiang Mai 50202, Thailand Received June 24, 2004
Two new dihydrostemofoline alkaloids, 11(S),12(R)-dihydrostemofoline (3) and stemoburkilline (4), along with stemofoline (1) and 2′-hydroxystemofoline (2) have been isolated from a root extract of Stemona burkillii Prain. The structure and relative configuration of 3 have been determined via spectroscopic data and from comparison with synthetic 11(S),12(S)-dihydrostemofoline (5). The configuration of the exo-cyclic alkene group in 4 is tentively assigned as E on the basis of mechanistic considerations. The Stemona group of alkaloids includes more than 40 different natural products that have been structurally classified into five different groups.1 The pyrrolo[1,2-a]azepine (5,7-bicyclic A,B-ring system) nucleus is common to all compounds in these groups. In 2003 we2 and then Hofer and Greger3 reported the structures of Stemona alkaloids with a pyrido[1,2-a]azepine A,B-ring system (that is, a 6,7-bicyclic A,B-ring system), and in 2004 we disclosed the structure of another pyrido[1,2-a]azepine Stemona alkaloid.4 These alkaloids comprise a new and sixth structural group. The pure alkaloids derived from the extracts of the leaves and roots of Stemona species have insect toxicity and antifeedent and repellent activities.3-5 We report here the isolation and structure determination of two novel Stemona alkaloids, 3 and 4, from the root extracts of Stemona burkillii Prain that were collected at Tambol Mae Hea, Amphur Meang, Chiang Mai, Thailand. A crude ethanol extract (10.4 g) of the roots of S. burkillii was partitioned between 5% hydrochloric acid solution and dichloromethane. The aqueous solution was made basic with aqueous ammonia and extracted with dichloromethane to afford 0.224 g of crude alkaloid material. Successive purifications of this material by preparative TLC gave pure samples of stemofoline 1 (6.8 mg), 2′-hydroxystemofoline 2 (3.7 mg), 11(S),12(R)-dihydrostemofoline 3 (2.1 mg), and stemoburkilline (4) (1.5 mg). The former two known alkaloids were identified from a comparison of their spectroscopic/spectrometric data (NMR and MS) with those reported.5,6 Compounds 3 and 4 are new compounds. We have named compound 4 stemoburkilline on the basis of its botanical origin. Examination of the crude ethanol extract by TLC and 1H NMR analysis showed the presence of all four alkaloids, indicating that these compounds were not being produced via an acid-catalyzed reaction during the acid extraction process. The HRMS (EI +ve, m/z [M]+ 389.2202, calcd 389.2202) of 3 showed it had the molecular formula C22H31NO5 and indicated that it was a dihydrostemofoline derivative. The 1H and 13C NMR specta of 3 indicated the presence of the A,B,C,D-ring system of stemofoline (1).5,6 However a comparison of the 13C/DEPT NMR spectra of 3 with that of 1 showed that 3 had two additional methine carbons (C-11 * To whom correspondence should be addressed. Tel: +61-24221-3511. Fax: +61-24221-4287. E-mail:
[email protected]. † University of Wollongong. ‡ Division of Environmental Sciences, Chiang Mai University. § Department of Biology, Chiang Mai University. ⊥ Department of Chemistry, Chiang Mai University.
10.1021/np049791z CCC: $27.50
[δ 86.3] and C-12 [δ 76.5]) and was missing the two quaternary carbons at δ 148.4 and 127.9 and for C-11 and
© 2004 American Chemical Society and American Society of Pharmacognosy Published on Web 08/28/2004
47.4 (CH2)
50.5 (CH) 111.8 (C)
47.3 (CH)
61.0 (CH)
33.1 (CH) 86.3 (CH)
76.5 (CH) 170.3 (C)
98.5 (C) 174.5 (C) 8.7 (CH3) 14.8 (CH3) 31.5 (CH2)
5a 5b 6a 6b 7 8
9
9a
10 11
12 13
14 15 16 17 1′a
23.2 (CH2)
13.9 (CH3) 58.8 (CH3)
4′ OMe
27.2 (CH2)
b 2′a b 3′
26.5 (CH2)
78.2 (CH) 82.2 (C)
2 3
δC (DEPT)
0.87(t, J ) 7) 4.11 (s)
1.40 (m) 1.23 (m) 1.33 (m)
2.01 (br s) 1.08 (d, J ) 6.5) 1.56 (t, J ) 8)
2.61 (m) 3.79 (dd, J10,11 ) 9, J11,12 ) 3) 4.60 (br s)
1.64 (dd, J9,9a ) 3, J9,10 ) 12) 3.44 (br s)
3.14 (m) R 3.01 (m) β 1.82 (m) 1.72 (m) 2.45 (d, J ) 6)
1.99 (m) 1.63 (dd, J1a,1b ) 3, J1b,2 ) 7.5) 4.22 (br s)
δH (mult., J (Hz), assign.
3
H-1′, H-2′a, H-2′b, H-4′ H-1′, H-2′b
H-1′, H3′, H-4′
H-1′, H-7, H-2′b, H-3′, H-4′
H-16 H-16
H-12, H-16, OMe
H-17 H-17
H-2, H-5b
H-7, H-10, H-17
H-1b, H-2, H-7
H-7 (w), H-5b (w)
H-1a, H-1′ H-1a, H-1b, H-1′
HMBC
14.1 (CH3) 59.3 (CH3)
23.7 (CH2)
27.5 (CH2)
99.1 (C) 170.5 (C) 8.7 (CH3) 18.7 (CH3) 30.2 (CH2)
141.9 (C) 161.8 (C)
28.4 (CH) 114.7 (CH)
63.4 (CH)
44.2 (CH)
55.4 (CH) 105.7 (C)
25.3 (CH2)
46.5 (CH2)
79.8 (CH) 82.9 (C)
32.9 (CH2)
δC (DEPT)
0.92 (t, J ) 6.8) 4.13 (s)
1.60 (m) 1.39 (m) 1.29 (m) 1.36 (m)
2.07 (s) 1.08 (d, J ) 6.8) 1.67 (m)
3.18 (m) 5.5 (d, J ) 10)
3.60 (br s)
1.85 (m)
2.34 (d, J ) 5.9)
3.27 (m) R 3.09 (m) β 1.93 (m)
4.38 (br s)
1.99 (m) 1.80 (m)
δH (mult., J (Hz), assign.
4 HMBC
H-3′
H-2′a, H-2′b, H-4′
H-4′ H-1′b, H-3′
H-10, H-11 H-2′b
H-16 H-16
H-10, H-11, H-16 H-11, H-16, OMe
H-7, H-10, H-11, H-17 H-2, H-5a, H-5b, H-9 H-9, H-17 H-10, H-17
H-6 H-6, H-7
H-7
H-1a, H-1′a H-1a, H-5b, H-1′a
NMR (125 Hz) and 1H NMR (500 Mz) Spectra Data for Compounds 3, 4, and 5 in CDCl3 Solution
33.4 (CH2)
13C
1a 1b
position
Table 1.
14.1 (CH3) 59.4 (CH3)
23.4 (CH2)
27.4 (CH2)
98.8 (C) 174.3 (C) 8.2 (CH3) 16.9 (CH3) 31.8 (CH2)
78.7 (CH) 173.3 (C)
35.1 (CH) 87.8 (CH)
61.1 (CH)
47.2 (CH)
50.5 (CH) 112.8 (C)
26.8 (CH2)
47.5 (CH2)
78.6 (CH) 82.1 (C)
33.4 (CH2)
δC (DEPT)
0.92 (t, J ) 6.8) 4.10 (s)
1.40 (m) 1.23 (m) 1.35 (q, J ) 6.8)
1.95 (br s) 1.12 (d, J ) 6.3) 1.54 (m)
4.75 (d, J ) 6.5)
2.48 (m) 3.69 (t, J ) 7)
3.38 (br s)
1.60 (m)
3.09 (m) R 2.96 (m) β 1.85 (m) 1.73 (m) 2.47 (d, J ) 6)
4.21 (br s)
1.97 (m) 1.62 (m)
δH (mult., J (Hz), assign.
5
H-3′
H-4′
H-3′, H-4′
H-11 H-7, H-3′, H-4′
H-10, H-16 H-11, H-12, H-16, OMe H-16 H-12, H-16
H-2, H-5a, H-5b, H-9 H-9, H-12, H-17 H-10, H-12, H-17
H-6b, H-1′ (w) H-2, H-6b, H-9, H-7, H-10, H-11 H-10, H-17
-
H-1b H-1a, H-5b, H-6b, H-7, H-1′ H-7
HMBC
Notes Journal of Natural Products, 2004, Vol. 67, No. 10 1741
1742 Journal of Natural Products, 2004, Vol. 67, No. 10
C-12, respectively, of stemofoline5,6 (Table 1). Furthermore, the 1H NMR spectrum of 3 showed two new signals at δ 3.79 (dd, J ) 3, 9 Hz, H-11) and 4.60 (br s, H-12), indicating that compound 3 was an 11,12-dihydrostemofoline. NOESY experiments showed a significant cross-peak between the C-10 methyl protons (H-17) and H-11, indicating their synrelationship. Thus, assuming that 3 had the same absolute configuration as stemofoline in the rings A-C, we have assigned the 11(S) configuration to compound 3. Unfortunately, these experiments did not permit assignment of the configuration at C-12. In 2003, Velten7 reported the synthesis of 11(S),12(S)-dihydrostemofoline 5 from the synhydrogenation of stemofoline. This compound also showed a significant cross-peak between the C-10 methyl protons (H-17) and H-11, consistent with the 11S configuration. Complete NMR data for 5 were, however, not reported. We have prepared compound 5 from hydrogenation of stemofoline 1, and the NMR data for this compound are shown in Table 1.7,8 The 1H and 13C NMR spectra of 3 and 5 are similar but not the same. Indeed, there is a significant difference in the chemical shifts and coupling constants for the signals for H-11 and H-12 in the 1H NMR spectra of these two compounds, especially J11,12, which was 3 Hz in 4 and 7 Hz in 5. On the basis of these differences we have assigned the 12R configuration to 3. The full 1H and 13C NMR spectra assignments for 3 and 5 based on extensive COSY, TOCSY, NOESY, HMQC, and HMBC experiments are shown in Table 1. A NOESY cross-peak between H-9 and H-5b permitted the unequivocal assignment of the H-5 protons (Table 1). The HRMS (EI +ve, m/z [M]+ 389.2194, calcd 389.2202) of stemoburkilline (4) showed that it also had the molecular formula C22H31NO5. Its 1H NMR spectrum indicated the presence of an olefinic proton (δ 5.5, 1H, d, J ) 10 Hz, H-11) coupled to an adjacent CH group (H-10), while its 13C/DEPT NMR spectrum, in comparison with that of 3, showed the C-11 and C-12 methines in 3 had been replaced by two olefinic carbons (one quaternary and one methine). The full 1H and 13C NMR spectra assignments for 4 based on extensive COSY, TOCSY, NOESY, HMQC, and HMBC experiments are shown in Table 1 and indicated that 4 was formally the C-ring opened product of 3. Our attempts to induce ring opening of 3 to produce 4 were not successful using either base (excess DBU, RT, 16 h) or acid (5% aqueous HCl, RT, 1 h) catalysis. The 13C NMR spectrum of 4 showed that this compound existed in the hemiacetal form (δ 105.7, C-8, quaternary), and this was further supported from its IR spectrum (3382 cm-1, br), which showed a hydroxyl group. NOESY experiments did permit assignment of the configuration of the C-11, C-12 alkene group. We have assigned the E configuration to 4 on the basis of the assumption that 4 arises from 3 via an antielimination process. Antifungal studies were done on the crude ethanol extract and on pure samples of 1 and 2 and mixtures of 1 and 2 and of 3 and 4. However these compounds and mixtures showed no significant activities (EC50 > 219 ppm) on inhibiting spore germination on Cladosporium cladosporiodes using the assay and procedures recommended in the literature.9 Brine shrimp assays10 on similar pure and mixed samples showed low to moderate toxicities (LC50 > 33 ppm). In conclusion, two new dihydrosteomofoline alkaloids, 11(S),12(R)-dihydrostemofoline (3) and stemoburkilline (4), along with stemofoline (1) and 2′-hydroxystemofoline (2) have been isolated from a root extract of S. burkillii. The structure and relative configuration of 3 have been deter-
Notes
mined by spectroscopic data interpretation and by comparisons with synthetic 11(S),12(S)-dihydrostemofoline (5), which was prepared by syn-hydrogenation of stemofoline (1). The configuration of the exo-cyclic alkene group in 4 could not be unequivocally determined and is tentatively assigned as E on the basis of mechanistic considerations. Experimental Section General Experimental Procedures. These were as described previously.2 Plant Material. The roots of S. burkillii were collected at Tambol Mae Hea, Amphur Meang, Chiang Mai, Thailand, in December 2003. The plant material was identified by Mr. James F. Maxwell from the Department of Biology, Chiang Mai University. A voucher specimen is deposited at the Herbarium (number 17579) of the Department of Biology, Chiang Mai University. Extraction and Isolation. The dry ground root of S. burkillii (1.8 kg) was extracted with 95% EtOH (3 × 2000 mL) over 3 days at room temperature. The EtOH solution was evaporated to give a dark residue (98 g). A portion of the extract (10.4 g) was partitioned between H2O and CH2Cl2. The CH2Cl2 extract was extracted with 5% HCl solution, and the aqueous solution was made basic with aqueous ammonia and extracted with CH2Cl2 to afford 0.224 g of crude alkaloid material. This material was chromatographed on silica gel (100 mL) using gradient elution from 100% CH2Cl2 to 10% MeOHCH2Cl2 containing 1% concentrated aqueous ammonia as eluent. A total of 900 mL of eluent was collected in test tubes of 20 mL. On the basis of TLC analysis these fractions were pooled to give two alkaloid fractions, fraction 1 (62 mg) and fraction 2 (88 mg). These fractions were further purified by preparative TLC. Separation of fraction 1 by three successive preparative TLC purifications (CH2Cl2-MeOH-aqueous ammonia, 97:3:1, then CH2Cl2-MeOH-aqueous ammonia, 98:2: 1, and then (CH2Cl2-EtOAc-MeOH-Et2NH, 70:30:5:1) gave pure samples of stemofoline (1) (6.8 mg) and 2′-hydroxystemofoline (2) (3.7 mg). Separation of fraction 2 by three successive preparative TLC purifications (CH2Cl2-MeOH-aqueous ammonia, 95:5:1, and then CH2Cl2-MeOH-aqueous ammonia, 96:4:1, and on TLC plates that were impregnated with NH4OAc using MeOH as eluent) gave pure samples of 11(S),12(R)-dihydrostemofoline (3) (2.1 mg) and stemoburkilline (4) (1.5 mg). The 1H and 13C NMR data of 1 and 2 were identical to that reported,5,6 while those of 3, 4, and 5 are shown in Table 1. Compound 3: yellow-brown gum; [R]26D +38.9° (c 0.35, CHCl3); IR (film) νmax 1753, 1671, 1458, 1389, 1339, 1233, 1216, 1079, 1031, 983 cm-1; HREI m/z 389.2202 [M+], calcd for C22H31NO5 389.2202. Compound 4 (stemoburkilline): yellow-brown gum; [R]26D +37.5° (c 0.28, CHCl3); IR (film) νmax 3382 (br), 1754, 1634, 1455, 1262, 1032, 987, 802 cm-1; HREI m/z 389.2195 [M+], calcd for C22H31NO5 389.2202. Hydrogenation of Stemofoline. To a solution of stemofoline (10.8 mg) in EtOH (1 mL) was added 10% Pd/C (3.7 mg). The mixture was left to stir under a hydrogen atmosphere (hydrogen balloon) at RT for 5 h, and then the reaction was filtered through a small pad of Celite and washed with more EtOH. The solvent was removed under reduced pressure, and the crude product was purified by preparative TLC (CH2Cl2EtOAc-MeOH-Et2NH, 70:30:5:1) to give compound 5 (5.3 mg) and an over-reduced product (2.5 mg).7 Compound 5: yellow gum; [R]26D +35.9 (c 0.22, CHCl3); IR (film) νmax 1754, 1668, 1636, 1458, 1391, 1339, 1061, 987 cm-1; HREIMS m/z 389.2201 [M]+, calcd for C22H31NO5 389.2202.
Note Added after ASAP: Structure 5 was incorrectly drawn in the version posted on August 28, 2004. The correct structure appears in the version posted on September 2, 2004. Acknowledgment. We are grateful to the National Research Council of Thailand (NRCT), the National Center for
Notes
Genetic Engineering and Biotechnology, Thailand (BIOTEC), and the University of Wollongong for supporting this project. We thank Dr. R. F. Velten, Bayer Crop Science AG, Leverkusen, Germany for sending us NMR data of compound 5. References and Notes (1) Pilli, R. A.; Ferreira de Oliveira, M. C. Nat. Prod. Rep. 2000, 17, 117127. (2) Mungkornasawakul, P.; Pyne, S. G.; Jatisatienr, A.; Supyen, D.; Lie, W.; Ung, A. T.; Skelton, B. W.; White, A. H. J. Nat. Prod. 2003, 66, 980-982. (3) Kaltenegger, E.; Brem, B.; Mereiter, K.; Kalchhauser, H.; Kahlig, H.; Hofer, O.; Vajrodaya, S.; Greger, H. Phytochemistry 2003, 63, 803816. (4) Mungkornasawakul, P.; Pyne, S. G.; Jatisatienr, A.; Supyen, D.; Jatisatienr, C.; Lie, W.; Ung, A. T.; Skelton, B. W.; White, A. H. J. Nat. Prod. 2004, 67, 675-677.
Journal of Natural Products, 2004, Vol. 67, No. 10 1743 (5) Brem, B.; Seger, C.; Pacher, T.; Hofer, O.; Vajrodaya, S.; Greger, H. J. Agric. Food Chem. 2002, 50, 6383-6388. (6) Seger, C.; Mereiter, K.; Kaltenegger, E.; Pacher, T.; Greger, H.; Hofer, O. Chem. Biodiversity 2004, 1, 265-279. (7) Ye, Y.; Velten, R. F. Tetrahedron Lett. 2003, 44, 7171-7173. (8) The NMR data of 5 prepared in our laboratory were almost identical to that of the data kindly sent to us by Dr. R. F. Velten, Bayer Crop Science AG, Leverkusen, Germany. (9) The American Phytopathological Society, Committee on Standardization of Fungicidal Tests. The slide-germination method of evaluating protectant fungicides. Phytopathology 1943, 33, 627-632. (10) (a) Teng, W. S. In Bioactive Natural Products: Detection, Isolation, and Structural Determination; Colegate, S. M., Molyneux, R. J., Eds.; CRC Press: Boca Raton, FL, 1993; Chapter 18, pp 441-456. (b) Meyer, B. N.; Ferrigni, N. R.; Putnam, J. E.; Jacobsen, L. B.; Nichols, D. E.; McLaughlin, J. L. Planta Med. 1982, 45, 31-34.
NP049791Z